Impaired biosynthesis of ergosterol confers resistance to complex sphingolipid biosynthesis inhibitor aureobasidin A in a PDR16-dependent manner

Complex sphingolipids and sterols are coordinately involved in various cellular functions, e.g. the formation of lipid microdomains. Here we found that budding yeast exhibits resistance to an antifungal drug, aureobasidin A (AbA), an inhibitor of Aur1 catalyzing the synthesis of inositolphosphorylceramide, under impaired biosynthesis of ergosterol, which includes deletion of ERG6, ERG2, or ERG5 involved in the final stages of the ergosterol biosynthesis pathway or miconazole; however, these defects of ergosterol biosynthesis did not confer resistance against repression of expression of AUR1 by a tetracycline-regulatable promoter. The deletion of ERG6, which confers strong resistance to AbA, results in suppression of a reduction in complex sphingolipids and accumulation of ceramides on AbA treatment, indicating that the deletion reduces the effectiveness of AbA against in vivo Aur1 activity. Previously, we reported that a similar effect to AbA sensitivity was observed when PDR16 or PDR17 was overexpressed. It was found that the effect of the impaired biosynthesis of ergosterol on the AbA sensitivity is completely abolished on deletion of PDR16. In addition, an increase in the expression level of Pdr16 was observed on the deletion of ERG6. These results suggested that abnormal ergosterol biosynthesis confers resistance to AbA in a PDR16-dependent manner, implying a novel functional relationship between complex sphingolipids and ergosterol.

the physiological importance of complex sphingolipids. The first and second steps of biosynthesis of sphingolipids are catalyzed by Lcb1 and Lcb2, serine palmitoyltransferase (SPT), and Tsc10, 3-ketodihydrosphingosine reductase, respectively (Fig. 1A), and these steps are essential for yeast, implying that depletion of all sphingolipids causes a lethal phenotype 3,4 . A lack of the Cer synthase gene (Lag1/Lac1) or their regulatory subunit Lip1 causes a severe growth defect but is not lethal, probably because trace level of biosynthesis of Cer still occurs via unknown mechanisms [5][6][7] . In yeast, there are three classes of complex sphingolipids, inositolphosphorylceramide (IPC), mannosylinositol phosphorylceramide (MIPC), and mannosyldiinositol phosphorylceramide (M(IP) 2 C), and the simplest structure of a complex sphingolipid is IPCs 1,2 (Fig. 1A). A lack of AUR1 encoding IPC synthase causes a lethal phenotype because of reductions in all the complex sphingolipid levels and accumulation of Cers 6,8 . In contrast, conversion of IPCs to MIPCs or MIPCs to M(IP) 2 Cs does not cause a cell growth defect, indicating that extension of the hydrophilic region of complex sphingolipids is not essential; however, biosynthesis of MIPCs is important for maintenance of endosomal trafficking, cell wall integrity, and acquisition of tolerance against multiple environmental stresses [9][10][11][12][13][14][15][16][17][18] .
Together with complex sphingolipids, ergosterol, a primary structure of sterol in budding yeast, is also an important constituent factor for formation of lipid microdomains 19 , and analyses of genetic interactions of genes involved in the biosynthesis of complex sphingolipids and ergosterol in yeast have indicated that these lipids function cooperatively. Comprehensive analysis of deletion of combinations of sphingolipid-metabolizing enzyme genes (SCS7, SUR2, and ISC1) and nonessential genes involved in the final steps of biosynthesis of ergosterol (ERG2, ERG3, ERG4, ERG5, and ERG6) revealed that simultaneous impairment of metabolism of sphingolipids and ergosterol causes multiple stress hypersensitivity 20 . Furthermore, synthetic lethal interaction due to deletion of ERG6 and ELO3 encoding an enzyme involved in biosynthesis of very long-chain fatty acids, that are used for sphingolipid biosynthesis, has also been reported 21 . In addition, impairment of cell wall integrity due to loss of biosynthesis of MIPCs is exacerbated by repression of expression of ERG9 encoding squalene synthase located in the middle stage of the ergosterol biosynthesis pathway 11 . Moreover, lethality caused by cumulative mutation of genes involved in ergosterol biosynthesis is suppressed by mutations causing alteration of the composition of complex sphingolipids 22 , supporting the notion of a close functional relationship between complex sphingolipids and ergosterol.
Aureobasidin A (AbA), a cyclic depsipeptide anti-fungal antibiotic isolated from a black-yeast-like fungus, Aureobasidium pullulans R106, inhibits the activity of Aur1 and has strong cytotoxic activity 8,23,24 . Several genes associated with determination of the sensitivity to AbA were identified, i.e. ATP-binding cassette transporters Pdr5 and Yor1 are involved in determination of AbA sensitivity, possibly by being indirectly or directly involved in the efflux of intracellularly accumulated AbA 25,26 . In addition, deletion of ELO3 confers resistance to AbA without affecting alteration of sphingolipid levels due to the AbA treatment 27 . The resistance due to the deletion of ELO3 is also observed when the expression level of AUR1 is repressed by a tetracycline-regulatable promoter, implying that the chain length of fatty acids in Cer are a critical factor determination of the cytotoxic activity of AbA 27 . This notion is also supported by the fact that the deletion of AUR1 does not cause a lethal phenotype when endogenous Cer synthases are replaced with one of the enzyme from cotton, in which Cers containing C18 fatty acids are produced instead of C26-Cers, the primary structure of Cers in wild-type budding yeast 28 .
In this study, we found that an impaired biosynthesis pathway for ergosterol, which is caused by the deletion of ERG6, ERG2, or ERG5, causes resistance to AbA; however, these effects are not observed under repression of expression of AUR1. The deletion of ERG6 results in suppression of reduction in complex sphingolipids and accumulation of Cers on the AbA treatment, indicating that the deletion reduces the effectiveness of AbA against in vivo Aur1 activity. Moreover, it was found that the acquisition of AbA resistance is mediated by PDR16, which was previously identified as a multicopy suppressor against AbA 29 . These results indicate a novel functional relationship between complex sphingolipids and ergosterol.

Results
Effects of a defect of the ergosterol biosynthesis pathway on the growth defect caused by impaired biosynthesis of sphingolipids. To investigate the functional relationship between sphingolipids and ergosterol, nonessential genes involved in the final stages of the ergosterol biosynthesis pathway (ERG2, ERG3, ERG4, ERG5, and ERG6) were deleted when sphingolipid biosynthesis was repressed by various means (Fig. 1C-G). To repress expression of AUR1 or LCB1, we used mutant strains that carry the AUR1 or LCB1 gene under the control of the tetracycline-regulatable (Tet) promoter (tet-AUR1 or tet-LCB1), and the expression was repressed by the addition doxycycline (Dox) 27 . Ptetoff-lip1-1 cells are also a strain that exhibits suppression of expression of LIP1 on the addition of Dox, but the ORF sequence in LIP1 contains a frameshift mutation, and thus the mutant cells exhibit a stronger inhibitory effect on Cer synthesis 30 . Under AUR1-repressive conditions, the cell growth defect phenotype was enhanced by the deletion of one of ERG2-6 ( Fig. 1C). The enhancement effect was also observed for erg2∆, erg3∆, erg5∆, or erg6∆ under LCB1-repressive conditions (Fig. 1D), and erg2∆, erg4∆, or erg6∆ under LIP1-repressive conditions (Fig. 1E). However, when cells were treated with aureobasidin A (AbA), an inhibitor of Aur1, the cell growth defect phenotypes were dramatically different from that observed on repression of expression of genes involved in sphingolipid metabolism; that is, the deletion of ERG2, ERG5, or ERG6 caused resistance to AbA (Fig. 1F). The effect of ERG2 or ERG6 on the AbA sensitivity was consistent with a previous report 31 . erg5∆ or erg6∆ cells, but not erg2∆ cells, also exhibited resistance to myriocin, an inhibitor of serine palmitoyltransferase; however, the effects were much weaker compared to that for AbA (Fig. 1F). Notably, treatment with miconazole, an inhibitor of lanosterol 14-alpha-demethylase, Erg11, at concentrations that do not induce a strong growth defect, also confers resistance to AbA (Fig. 1H). Thus, it was suggested that impaired biosynthesis of ergosterol confers resistance to AbA.  (Fig. 1F).   Fig. S1, abnormal cell morphology that was observed in AbA-treated wild-type cells did not seem to be observed in erg6∆ cells. Moreover, the appearance of propidium iodide (PI)-positive cells in the presence of AbA was greatly suppressed by the deletion of ERG6, suggesting suppression of cell death (Fig. S2). Inhibition of the activity of Aur1 causes both reductions in complex sphingolipid levels and accumulation of Cers, both of which are believed to lead to a cell growth defect caused by the inhibition 6,8 . Thus, we next investigated whether or not erg6∆ affects the alteration of complex sphingolipid and Cer levels caused by the AbA treatment. Figure 2A shows the time courses for cells in the presence of AbA. The growth of wild-type cells began to be delayed at around 5 h after the addition of 50 ng/ml of AbA; however, the delay was dramatically attenuated by the deletion of ERG6. Thus, we decided to measure the complex sphingolipid and Cer levels at 5 and 8 h after the addition of 50 ng/ml of AbA. As reported previously, AbA treatment of wild-type cells caused a significant reduction in the level of complex sphingolipids; however, in erg6∆ cells, such reduction was not observed (Fig. 2B,D). The accumulated level of Cer-C due to the AbA treatment was dramatically suppressed by the deletion of ERG6 (Fig. 2C,E). These results indicated that the inhibitory effects of AbA on biosynthesis of IPCs is suppressed on the deletion of ERG6. We also examined the effect of erg6∆ on alteration of sphingolipid levels by repression of expression of AUR1 by the Tet promoter. As in the spot assay (Fig. 1C), in liquid culture, the deletion of ERG6 also did not confer resistance to repression of expression of AUR1 in the presence of 2 or 10 µg/ ml of Dox (Fig. 2F). As shown in Fig. 2G, the reduction in complex sphingolipid levels was indistinguishable between Dox-treated tet-AUR1 and tet-AUR1 erg6∆ cells.
To confirm the effect of erg6∆ on in vivo inhibitory activity of AbA toward Aur1, C6-NBD-Cer was used. Exogenously added C6-NBD-Cer is incorporated into yeast cells and converted to C6-NBD-IPC 32,33 . As shown in Fig. 3A, production of C6-NBD-IPC in wild-type and erg6∆ cells was inhibited by addition of AbA in a concentration-dependent manner; however, the effectiveness of AbA in erg6∆ cells was much weaker than that in wild-type cells. In contrast, the inhibitory effect of AbA on IPC synthase activity in cell lysates did not differ between wild-type and erg6∆ cells (Fig. 3B). Thus, it was suggested that the resistance to AbA due to erg6∆ is caused by reduced effectiveness of AbA against in vivo Aur1 activity.
One possibility is that the deletion of ERG6 causes an increase in the protein expression level of IPC synthase, and thus reduces the efficiency of AbA; however, the protein expression levels of Aur1 and Kei1 (an essential component of IPC synthase 34 ) were not significantly different between wild-type and erg6∆ cells when chromosomal AUR1 and KEI1 were tagged with a sequence encoding six copies of the hemagglutinin (HA) epitope (6xHA), and the tagged proteins were detected with an anti-HA antibody (Fig. 3C) 17 . In addition, in tet-AUR1 cells, which exhibit constitutive expression of AUR1 due to the Tet-promoter in the absence of Dox, the deletion of ERG6 also conferred the AbA resistance (Fig. 3D), supporting the notion that erg6∆ does not cause resistance to AbA through altered activity of the native promoter of AUR1. It has been reported that Aur1 is localized at the medial Golgi 32 , and we confirmed that Aur1-eqFP611 is colocalized with the medial Golgi marker yeGFP-Gos1 (Fig. 3E) 35 . This colocalization was not altered by the deletion of ERG6 (Fig. 3E). Thus, it was suggested that the deletion of ERG6 affects the effectiveness of AbA against in vivo Aur1 activity without alteration of the protein expression level and subcellular localization of Aur1. To examine whether or not the deletion of ERG6 affects the incorporation of AbA into cells, the intracellular level of AbA in cells treated with 50 or 100 ng/ml AbA for 1 h was determined by LC-ESI MS/MS. As shown in Fig. 3F, a significant difference in the intracellular AbA level between AbA-treated wild-type and erg6∆ cells was not observed.
Resistance to AbA due to impaired biosynthesis of ergosterol is caused in a PDR16-dependent manner. Previously, we reported that overexpression of PDR16 or PDR17, which encode proteins belonging to the phosphatidylinositol transfer protein family (PITP family) 36 , confers resistance to AbA; however, the overexpression does not suppress the growth defect caused by the AUR1 repression 29 . Thus, we next investigated the relationship between ERG6 and PDR16/17 on determination of the AbA sensitivity. As shown in Fig. 4A, the AbA resistance due to erg6∆ was completely abolished on deletion of PDR16 (erg6∆ versus erg6∆ pdr16∆ cells); however, the AbA sensitivity in wild-type and pdr16∆ cells was indistinguishable. Reduced resistance to Cells were cultured overnight in YPD medium, diluted (0.05 OD 600 units/ml) in fresh YPD medium, and incubated for 3 h at 30 °C, and then the indicated concentration of AbA was added to the culture. Aliquots of cell suspensions were subjected to cell density measurements (OD 600 ) at the indicated times. (B-E) TLC analysis of complex sphingolipids and Cer-C. Cells were cultured overnight in YPD medium, diluted (0.05 OD 600 units/ml) in fresh YPD medium, incubated for 3 h at 30 °C, and then treated with 0 or 50 ng/ml AbA for 5 or 8 h at 30 °C. Lipids were extracted, and then separated by TLC. Complex sphingolipids and Cer-C were quantified with IMAGEJ software (NIH). The amounts of complex sphingolipids (IPCs, MIPCs, and M(IP) 2 Cs) (B,D) and Cer-C (C,E) in AbA-untreated wild-type cells were taken as 1, respectively. The original TLC plates are presented in Fig. S11A. (F) Time course of growth of AUR1-repressed cells. Cells were cultured overnight in YPD medium, diluted (0.018 OD 600 units/ml) in fresh YPD medium, and incubated for 3 h at 30 °C, and then the indicated concentration of Dox was added to the culture. Cell density at the indicated times was measured as described in (A). (G) Cells were cultured overnight in YPD medium, diluted (0.018 OD 600 units/ml) in fresh YPD medium, incubated for 3 h at 30 °C, and then treated with 10 µg/ml Dox for 15 h at 30 °C. TLC analysis was performed as described in (B). The amounts of complex sphingolipids (IPCs, MIPCs, and M(IP) 2 Cs) in Dox-untreated tet-AUR1 cells were taken as 1, respectively. The original TLC plate is presented in Fig. S11A. Data represent means ± SD from one experiment (triplicate) representative of three independent experiments. The details are given in "Methods". www.nature.com/scientificreports/ AbA was also observed on deletion of PDR17 (erg6∆ versus erg6∆ pdr17∆ cells); however, this effect is much weaker than that of PDR16 (Fig. 4A). Thus, it was suggested that Pdr16 contributes to the AbA resistance of erg6∆ cells much more than Pdr17. It should be noted that erg6∆ pdr16∆ cells exhibited higher AbA sensitivity than wild-type and pdr16∆ cells (Fig. 4A). Furthermore, under our experimental conditions, pdr17∆ cells exhibited higher AbA sensitivity than wild-type cells (Fig. 4A). In contrast, as compared with effects of deletion of PDR16 or PDR17 on ERG6-deleted cells treated with AbA, the deletion of PDR16 or PDR17 had only a weak effect on cell growth of ERG6-deleted tet-AUR1 cells in the presence of Dox (Dox-treated tet-AUR1 erg6∆ versus Dox-treated tet-AUR1 erg6∆ pdr16∆ or tet-AUR1 erg6∆ pdr17∆ cells) (Fig. 4B). The AbA resistance due to the deletion of ERG2 or ERG5 or treatment with miconazole was also abolished on the deletion of PDR16 (Fig. 4C,D), suggesting that the acquisition of resistance to AbA due to the impaired biosynthesis of ergosterol  www.nature.com/scientificreports/ biosynthesis depends on PDR16. Sensitivity to myriocin was also suppressed by the deletion of ERG5 or ERG6 (Fig. 1G); however, pdr16∆ slightly suppressed but did not completely abolish the myriocin resistance due to erg5∆ or erg6∆ (Fig. S3). Plasma membrane-localized ABC transporters are involved in attenuation of the cytotoxic effects of various drugs, and Pdr5 and Yor1 are involved in determination of sensitivity to AbA 25,26 . Thus, we also examined whether or not the AbA resistance due the deletion of ERG6 is affected by deletion of genes encoding plasma membrane localized-ABC transporters with known functions (AUS1, SNQ2, PDR10, PDR11, PDR12, PDR15, PDR5, YOR1, PDR18, and STE6) 37 (Fig. 4E). The deletion of PDR5 or YOR1 slightly altered the www.nature.com/scientificreports/ AbA sensitivity of ERG6-deleted cells; however, strong AbA resistance was still observed. For other genes, notable effects were not observed in ERG6-deleted cells (Fig. 4E). Figure 5 shows the effects of deletion of PDR16 and/or PDR17 on alteration of complex sphingolipid and Cer-C levels due to the AbA treatment. Although the deletion of ERG6 caused suppression of reduction in complex sphingolipid levels and accumulation of Cer-C levels in the presence of AbA (wild-type versus erg6∆ cells), no significant differences in sphingolipid levels were observed between AbA-treated pdr16∆ and pdr16∆ erg6∆ cells (Fig. 5A,B). The deletion of PDR17 also suppressed the effect of ERG6 (pdr17∆ versus pdr17∆ erg6∆ cells); however, the effect was much weaker than that of PDR16 (Fig. 5A,B). These results are consistent with the tendency seen in the AbA sensitivity (Fig. 4A). The effect of double deletion of PDR16 and PDR17 on ERG6-deleted cells was similar to that of single deletion of PDR16; that is, no significant differences were observed between pdr16∆ pdr17∆ and pdr16∆ pdr17∆ erg6∆ cells in the alterations of sphingolipid levels due to AbA treatment (Fig. 5C,D). Thus, it was suggested that deletion of PDR16 alone is sufficient to counteract the suppressive effect of AbA on the deletion of ERG6.
Increase in the expression level of Pdr16 in ERG6-deleted cells. It is possible that the deletion of ERG6 increases the expression level of Pdr16 and/or Pdr17 and thus confers the AbA resistance. Thus, we next examined the protein expression level of Pdr16 and Pdr17 in wild-type and erg6∆ cells. For detection of Pdr16 and Pdr17 by Western blotting, the chromosomal PDR16 and PDR17 were tagged with a sequence encoding 6xHA 29 . erg6∆ cells exhibited an approximately 25% increase in the protein expression level of Pdr16-6xHA as compared with wild-type cells; however, no significant difference in that of Pdr17-6xHA was observed between wild-type and erg6∆ cells (Fig. 6A). AbA treatment for 3 or 6 h did not cause a notable change in the Pdr16-6xHA and Pdr17-6xHA expression levels regardless of the ERG6 deletion (Fig. S4). The increase in the expression level of Pdr16 due to erg6∆ was also observed when the chromosomal PDR16 was tagged with a sequence encoding yeGFP (Fig. 6B,C). When the promoter region of chromosomal PDR16 was replaced by the ADH or CYC1 promoter, the increase in the expression level of Pdr16-yeGFP due to erg6∆ was still observed (Fig. 6C). Moreover, the promoter activity of PDR16 was not increased, but rather slightly decreased, on the deletion of ERG6 when a reporter gene plasmid, which contains a potential promoter region of PDR16 and the alpha-galactosidase gene, was used for the estimation (Fig. 6D). These results suggested that the increase in the protein expression level of Pdr16 due to erg6∆ occurs posttranslationally. When Pdr16 was expressed under the control of the CYC1 promoter, the deletion of ERG6 caused resistance to AbA (CYC1p-PDR16 versus CYC1p-PDR16 erg6∆ cells) (Fig. 6E). Moreover, CYC1p-PDR16 erg6∆ cells were more resistant to AbA than wild-type cells even though the expression level of Pdr16-yeGFP with the CYC1 promoter is much lower than that with the native promoter (Fig. 6C,E), implying that the mechanism of PDR16-mediated AbA resistance acquisition in the ERG6-deleted cells is not solely due to the increased Pdr16 expression level. ADHp-PDR16 erg6∆ cells were more resistant to AbA than wild-type cells; however, the resistance was weaker than that of erg6∆ cells even though the expression level of Pdr16-yeGFP with the ADH promoter is higher than that with the native promoter (Fig. 6C,E). This suggested that excessive Pdr16 overexpression is rather detrimental to the ERG6-deleted cells. Pdr16 is primarily localized to the cytosol and lipid droplets, but it has been reported that it is preferentially localized to the lipid droplets close to nucleus-vacuole junctions (NVJs) 38 . When lipid droplets were stained with Nile red, localization of Pdr16-yeGFP to lipid droplets was observed in both wild-type and ERG6-deleted cells (Fig. 6F). Moreover, in both the wild-type and ERG6-deleted cells, Pdr16-yeGFP was localized to the lipid droplets close to eqFP611-tagged Nvj1 that is involved in formation of NVJ (Fig. 6G) 38 . In addition, colocalization of Aur1-yeGFP and Pdr16-eqFP69 was not observed in both wild-type and erg6∆ cells (Fig. S5). These results suggested that the localization pattern of Pdr16 is not affected by the deletion of ERG6.

Discussion
In this study, it was found that impaired biosynthesis of ergosterol, which includes deletion of ERG6, ERG2, or ERG5 or treatment with miconazole, causes Pdr16-mediated resistance to AbA. Among PITP family proteins (Sec14, Sfh1, Csr1, Pdr16, Pdr17, and Sfh5), only Pdr16 and Pdr17 confer strong resistance to AbA when each protein is overexpressed 29 ; however, the suppressive effect of pdr17∆ on the AbA resistance caused by erg6∆ was much weaker than that of pdr16∆ (Figs. 4A and 5A,B). Moreover, the suppressive effects of erg6∆ on reductions in complex sphingolipid levels and accumulation of Cer-C in the presence of AbA was almost completely abolished by pdr16∆ (wild-type or pdr16∆ cells versus erg6∆ pdr16∆ cells) (Fig. 5A,B), and the effect of double deletion of PDR16 and PDR17 on the alteration of sphingolipid levels by AbA was comparable to that of single deletion of PDR16 (Fig. 5). Thus, it is suggested that Pdr16 plays a main role in acquisition of AbA resistance due to erg6∆. However, single deletion of PDR17 has a weak effect on ERG6-deleted cells, suggesting that Pdr17 is required for Pdr16 to be fully effective in the AbA resistance. It should be noted that a notable difference of AbA sensitivity was not observed between wild-type and pdr16∆ cells (Fig. 4A), implying that Pdr16 confers AbA resistance only when ergosterol biosynthesis is impaired or Pdr16 is overexpressed.
In ERG6 cells, deletion of PDR17 (also double deletion of PDR16 and PDR17), but not that of PDR16 alone, enhanced the growth defect in AbA-treated cells (Fig. 4A); however, alteration of sphingolipid levels caused by AbA was not affected by pdr17∆ or pdr16∆ pdr17∆ (wild-type versus pdr17∆ or pdr16∆ pdr17∆ cells) (Fig. 5). This suggests that Pdr17 (possibly also Pdr16) affects the growth defect caused by abnormal metabolism of complex sphingolipids, in addition to affecting the effectiveness of AbA against in vivo Aur1 activity. This notion is also supported by the fact that, in tet-AUR1 cells, the deletion of PDR17 (also double deletion of PDR16 and PDR17) also enhanced the growth defect on the addition of Dox (Fig. 4B). Since Pdr17 and Pdr16 bind to phosphatidylinositol and facilitate transfer of this lipid between membranes 36 , the possibility should be considered that Pdr17/16 directly interact with complex sphingolipids and/or Cers, and the deletion of PDR17/ 16   www.nature.com/scientificreports/ is involved in transport of phosphatidylserine from the ER to endosomes, and affects the efficiency of conversion of phosphatidylserine to phosphatidylethanolamine catalyzed by endosome-localized Psd2 39,40 . It should be noted that, under AUR1-repressive conditions, the phosphatidylserine and phosphatidylethanolamine levels are decreased 41 . Thus, it is also important to consider that the function of Pdr17 in phosphatidylserine metabolism affects the growth defect on impairment of metabolism of complex sphingolipids. It has been suggested that Pdr16 and Pdr17 are also involved in the metabolism and transport of sterols. The deletion of PDR16 and/or PDR17 causes a reduction in the ergosterol level and accumulation of its synthetic intermediates 42 . Furthermore, very recently, it was reported that, in an in vitro assay, Pdr16 and Pdr17 facilitate transfer of lanosterol, an ergosterol precursor, between membranes 43 . Therefore, it would be important to investigate whether or not the functions of Pdr16 and Pdr17 in sterol metabolism and transport are involved in In ERG6-deleted cells, the protein expression level of Pdr16, but not that of Pdr17, was posttranslationally upregulated (Fig. 6), and thus it is assumed that an increased level of Pdr16 is one of the factors leading to the acquisition of AbA resistance via Pdr16. However, when PDR16 was expressed under the CYC1 promoter, ERG6deleted cells exhibited very weak resistance to AbA as compared with wild-type cells (Wild-type cells versus CYC1p-PDR16 erg6∆ cells) (Fig. 6E), although the expression of Pdr16 under the CYC1 promoter was lower than that under the native promoter even when ERG6 was deleted (Fig. 6C). This suggests that the deletion of ERG6 contributes to Pdr16-mediated acquisition of AbA resistance through unknown mechanism(s), in addition to induction of an increase in the Pdr16 expression level. There were no notable differences in localization of Pdr16 to lipid droplets between ERG6 and erg6∆ cells (Fig. 6F,G). Deletion of ERG6, ERG2, or ERG5 causes accumulation of the synthetic intermediate instead of ergosterol, and the total amount of sterols is not reduced 20 . It is possible that this alteration of sterol composition changes characteristic of lipid droplets, which may result in an increase in the AbA resistance-conferring activity of Pdr16 localized to lipid droplets. In particular, the fact that Erg6 is localized not only in the ER but also in lipid droplets may be related to the strong AbA resistance conferred by erg6∆ 44 .
How does Pdr16 confer resistance to AbA? It was reported that deletion of PDR5 or double deletion of PDR5 and YOR1, which encode plasma membrane-localized ABC transporters, confers resistance to AbA, possibly by regulating the permeability of AbA across plasma membranes 26,31 . In addition, single deletion of YOR1 causes AbA hypersensitivity 25 . However, the deletion of ERG6 did not affect incorporation efficiency of AbA into cells (Fig. 3F). Furthermore, deletion of PDR5 enhanced the AbA resistance in ERG6-deleted cells (erg6∆ versus erg6∆ pdr5∆ cells), and erg6∆ yor1∆ cells still exhibited the AbA resistance as compared with wild-type cells (Fig. 4E), suggesting that the AbA resistance conferred by the deletion of ERG6 is independent from Pdr5 and Yor1. One hypothesis is that Pdr16 restricts the accessibility of AbA to Aur1 by trapping AbA, and confers the AbA resistance without affecting incorporation efficiency of AbA into cells. Mutation of Asp235 and Lys267, which are important residues for the phosphatidylinositol binding activity of Pdr16, abolishes the AbA resistance-conferring activity of Pdr16 29,45 , suggesting the importance of the lipid binding site for acquisition of AbA resistance. Therefore, evaluation of the interaction between the lipid binding site of Pdr16 and AbA may be an important issue when assessing the mechanism of conferring AbA resistance mediated by Pdr16. On the other hand, PDR16-deleted cells exhibit hypersensitivity to azole compounds, and expression of Pdr16, but not Pdr16-E235A, K267A, in the pdr16∆ cells can complement the azole hypersensitivity 45 . Furthermore, Pdr16 reduces the inhibitory effect of azoles against the in vivo activity of Erg11, a target of azoles; however, it does not affect the efficiency of uptake of azoles into cells 46 , which is consistent with the fact that erg6∆ did not affect the uptake of AbA (Fig. 3F). Thus, these findings may suggest a common mechanism that confers resistance to AbA and azoles via Pdr16.
This study indicates a new connection between sphingolipids and ergosterol; that is, a growth defect caused by repression of expression of AUR1, LCB1, or LIP1 is enhanced by impairment of the ergosterol biosynthesis pathway (Fig. 1), implying that simultaneous abnormal metabolism of sphingolipids and ergosterol has more profound effects on cell growth, whereas the impairment of ergosterol confers resistance to AbA through affecting the effectiveness of this inhibitor against in vivo Aur1 activity. Based on these results, it is assumed that, in order to avoid the risk of a simultaneous defect of ergosterol and sphingolipid metabolism, yeast may acquire AbA resistance through Pdr16 under the conditions of impaired biosynthesis of ergosterol. Complex sphingolipids and ergosterol function together in the formation of lipid microdomains 19 , and it should be noted that Can1 Figure 6. Effects of deletion of ERG6 on the protein expression level and localization of Pdr16. (A) Protein expression levels of Pdr16 and Pdr17. Cells expressing Pdr16-6xHA or Pdr17-6xHA with the native promoter were cultured overnight in YPD medium, diluted (0.3 OD 600 units/ml) in fresh YPD medium, and then incubated for 5 h at 30 °C. Yeast cell extracts were immunoblotted using anti-HA or anti-Pgk1. The amount of each tagged protein in ERG6 cells was taken as 1. Data represent means ± SD from one experiment (triplicate) representative of three independent experiments. The original blots are presented in Fig. S8. (B) Cells expressing Pdr16-yeGFP were cultured as described in (A). GFP fluorescence was observed by fluorescence microscopy. (C) Expression of PDR16-yeGFP by the native promoter, CYC1 promoter, or ADH promoter. Cells were cultured as described in (A). Fluorescence intensity of GFP in individual cells was measured with a flow cytometer. Each value is the average of the fluorescence intensity of 10,000 cells from one sample. The fluorescence intensity in PDR16-yeGFP cells was taken as 1. Data represent means ± SD for three samples representative of three independent experiments. (D) Promoter activity of PDR16. Cells harboring pRS415-PDR16p-MEL1 were cultured overnight in SC medium lacking leucine (SC-LEU), diluted (0.3 OD 600 unit/ml) in fresh SC-LEU medium, and then incubated for 5 h at 30 °C. Cells were harvested and alpha-galactosidase activity was measured as described under "Methods". Data represent means ± SD from one experiment (triplicate) representative of three independent experiments. (E) Effect of erg6∆ on AbA sensitivity of cells expressing PDR16 via the native promoter, CYC1 promoter, or ADH promoter. Cells cultured overnight in YPD medium were spotted onto YPD plates with or without the indicated concentrations of AbA. (F) Nile red staining of cells expressing Pdr16-yeGFP. Cells were cultured as described in (A), stained with 5 µg/ml of Nile red for 20 min, washed with water, and then observed by fluorescence microscopy. (G) Cells expressing Pdr16-yeGFP and Nvj1-eqFP611 were cultured as described in (A). GFP and RFP fluorescence was observed by fluorescence microscopy. The details are given in "Methods". www.nature.com/scientificreports/ and Tat2, which are suggested to localized at lipid microdomains 47 , were slightly increased by the deletion of ERG6, which may suggest some abnormality in lipid microdomains in erg6∆ cells (Fig. S6). Further analysis as to the molecular mechanism underlying the AbA resistance-conferring activity of Pdr16 under impaired biosynthesis of ergosterol will provide a deeper insight into the drug-resistance mechanism and relationship between sphingolipids and sterols.

Methods
Yeast strains and media. The S. cerevisiae strains used are listed in Table 1. Disruption of genes was performed by replacing their open reading frames with the kanMX4 marker from pFA6a-kanMX4, the hphNT1 marker from pFA6a-hphNT1, or the natNT2 marker from pFA6a-natNT2 48 . For expression of genes by a constitutive ADH or CYC1 promoter, a ADH or CYC1 promoter cassette containing the kanMX4 marker from pYM-N6 or pYM-N10, respectively, was introduced immediately upstream of the initiator ATG of the chromosomal gene, as described previously 48 . BY4741 cells having Ptetoff-lip1-1 were obtained by replacing the LIP1 gene with Ptetoff-lip1-1::HIS3MX6 derived from DYY1 cells (SEY6210.1, Ptetoff-lip1-1::HIS3MX6 30 ). For tagging of the C-terminus of Aur1, Pdr16, or Nvj1 with a yeast enhanced green fluorescent protein (yeGFP) or a red fluorescence protein (eqFP611), a yeGFP fusion cassette with the hphNT1 marker from pYM25 or a eqFP611 fusion cassette with the kanMX4 marker from pYM51 was introduced immediately upstream of the stop codon of each chromosomal gene as described previously 30 . For tagging of the N-terminus of Gos1 with a yeast yeGFP tag, a yeGFP fusion cassette with the ADH promoter and natNT2 marker from pYM-N9 was introduced immediately downstream of the initiator ATG of chromosomal GOS1 as described previously 30 . The cells were cultured in YPD medium (1% yeast extract, 2% peptone and 2% glucose), or SC (synthetic complete) medium (0.67% yeast nitrogen base without amino acids (BD Difco, Heidelberg, Germany) and 2% glucose) containing nutritional supplements. The lipid extracts were centrifuged at 10,000g for 1 min and then extracted once more in the same manner. The resulting supernatants were dried and the residue was dissolved in 130 μl monomethylamine (40% methanol solution)/water (10:3, v/v), followed by incubation for 1 h at 53 °C (mild alkaline treatment). The samples were dried, suspended in 60 µl of chloroform/methanol/ water (5:4:1, v/v), and then separated on Silica Gel 60 TLC plates (Merck, Whitehouse Station, NJ) with chloroform/methanol/4.2 M ammonia (9:7:2, v/v) (for detection of complex sphingolipids) or chloroform/methanol/ acetic acid (100:6:0.6, v/v) (for detection of Cer-C) as the solvent system. The TLC plates were sprayed with 10% copper sulphate in 8% orthophosphoric acid and then heated at 180 °C to visualize lipids. Identification of each complex sphingolipid and Cer-C was performed as described in previous papers 27,50 .

Incorporation of C6-NBD-Cer into cells. Cells treated with C6-NBD-Cer (Thermo Fisher Scientific,
Waltham, MA, USA) were collected by centrifugation and then washed with ice-cold YPD medium containing 1 mg/ml of fatty acid-free BSA. The cell pellets were washed twice with ice-cold water, and lipids were extracted as described above (except for the mild alkaline treatment), and then separated on TLC plates with chloroform/ methanol/4.2 M ammonia (9:7:2, v/v) as described in above. The fluorescent lipids were visualized with Omega Lum G (Aplegen; Pleasanton, CA, USA) and quantified with ImageJ software. Measurement of in vitro IPC synthase activity. Cells (10 OD 600 units) were suspended in 1 ml of 100 mM Tris-HCl buffer, pH 9.4, containing 0.28% 2-mercaptoethanol, incubated at room temperature for 10 min, and then collected by centrifugation. Cells were resuspended in 2 ml of 40 mM Tris-HCl buffer, pH 7.5, containing 1.2 M sorbitol and 50 µg/ml of zymolyase 20T (Nacalai Tesque, Kyoto, Japan), incubated at 30 °C for 30 min, and then collected by centrifugation. Spheroplasts were lysed by sonication in 1 ml of buffer A (5 mM Tris-HCl buffer, pH 7.5, containing 150 mM NaCl, 1 mM EDTA, and 1 × protease inhibitor mixture (Complete™ EDTA free; Roche Applied Science)). After removal of cell debris by centrifugation at 1000g for 3 min at 4 °C, the protein content of the supernatant was determined by the bicinchoninic acid method (Takara Bio, Shiga, Japan). One nmol of C6-NBD-Cer, 5 µg of phosphatidylinositol from soybeans (Nacalai Tesque), and 0, 0.12, or 0.36 ng of AbA were added to a cell lysate containing 20 µg of cell protein in 120 µl of buffer A. Following incubation at 30 °C for 30 min, the reaction was terminated by the addition of 500 µl of chloroform/methanol (2/1, v/v). The resultant organic phase was dried, and NBD-lipids were separated on TLC plates and quantified as described in above.

Yeast protein extraction, SDS-PAGE and western blotting. Protein extraction, SDS-PAGE and
Western blotting were performed as described elsewhere 51 with some modifications. For protein extraction, yeast cells grown in YPD medium were collected by centrifugation, washed with water, and then resuspended in 100 µl of 0.2 N NaOH containing 0.5% 2-mercaptoethanol. Each suspension was incubated on ice for 15 min. One ml of ice-cold acetone was added to the suspension, followed by incubation for 30 min at − 25 °C, and then the proteins were precipitated by centrifugation for 10 min at 10,000g. The pellet was resuspended in 100 µl of SDS sample buffer (156 mM Tris-HCl, pH 6.8, containing 5% SDS, 25% glycerol, 5% 2-mercaptoethanol and 0.001% bromophenol blue). The suspension was mixed well, heated for 3 min at 95 °C, and then centrifuged for 1 min at 10,000g. Then the supernatant was separated by SDS-PAGE according to the method of Laemmli 52 . For Western blotting, anti-HA (Sigma-Aldrich), and anti-Pgk1 (Thermo Fisher Scientific) were used as primary antibodies. Horseradish peroxidase-conjugated anti-mouse IgG (Thermo Fisher Scientific) was used as the secondary antibody.
Briefly, cells (2 OD 600 U) were suspended in 200 µl of 20 mM Tris-HCl buffer, pH 7.5, containing 0.35% 2-mercaptoethanol and 0.002% SDS, 5 µl of chloroform was added, and then the samples were vortexed for 10 s. After 5 min pre-incubation at 30 °C, the samples (200 µl) were mixed with 80 µl of 7 mM p-nitrophenyl-α-galactoside (Sigma-Aldrich, St. Louis, MO, USA) in 100 mM citric acid buffer, pH 4.0, and then incubated at 30 °C for 1 h. Following quenching of the reaction with 900 µl of 0.1 M NaOH, samples were centrifuged at 10,000g for 1 min, and the absorbance at 410 nm of the supernatants was measured.
Statistical analysis. Statistical analysis was performed using Student's t test, and the P values obtained are indicated.

Data availability
The datasets used and/or analysed during the current study available from the corresponding author on reasonable request.